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Laminin-5 and type I collagen promote adhesion and osteogenic differentiation of animal serum-free expanded human mesenchymal stromal cells

机译:层粘连蛋白5和I型胶原蛋白促进动物无血清扩增的人间充质基质细胞的粘附和成骨分化

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摘要

Mesenchymal stromal cells (MSC) are differentiation competent cells and may generate, among others, mature osteoblasts or chondrocytes in vitro and in vivo. Laminin-5 and type I collagen are important components of the extracellular matrix. They are involved in a variety of cellular and extracellular activities including cell attachment and osteogenic differentiation of MSC. MSC were isolated and expanded using media conforming good medical practice (GMP)-regulations for medical products. Cells were characterized according to the defined minimal criteria for multipotent MSC. MTT- and BrdU-assays were performed to evaluate protein-dependent (laminin-5, laminin-1, type I collagen) metabolic activity and proliferation of MSC. MSC-attachment assays were performed using protein-coated culture plates. Osteogenic differentiation of MSC was measured by protein-dependant mineralization and expression of osteogenic marker genes (osteopontin, alkaline phophatase, Runx2) after three, seven and 28 days of differentiation. Marker genes were identified using quantitative reverse-transcription polymerase chain reaction. Expansion of MSC in GMP-conforming media yielded vital cells meeting all minimal criteria for MSC. Attachment assay revealed a favorable binding of MSC to laminin-5 and type I collagen at a protein concentration of 1–5 fmol/µL. Compared to plastic, osteogenic differentiation was significantly increased by laminin-5 after 28 days of culture (P<0.04). No significant differences in gene expression patterns were observed. We conclude that laminin-5 and type I collagen promote attachment, but laminin-1 and laminin-5 promote osteogenic differentiation of MSC. This may influence future clinical applications.
机译:间充质基质细胞(MSC)是分化能力细胞,在体外和体内均可产生成熟的成骨细胞或软骨细胞。层粘连蛋白5和I型胶原蛋白是细胞外基质的重要组成部分。它们参与多种细胞和细胞外活动,包括细胞附着和MSC的成骨分化。使用符合医疗产品质量管理规范(GMP)规定的培养基分离和扩增MSC。根据多能MSC定义的最低标准对细胞进行表征。进行了MTT和BrdU分析以评估蛋白质依赖性(laminin-5,laminin-1,I型胶原)代谢活性和MSC的增殖。使用蛋白包被的培养板进行MSC附着测定。在分化三天,七天和二十八天后,通过蛋白质依赖性矿化作用和成骨标记基因(骨桥蛋白,碱性磷酸酶,Runx2)的表达来测量MSC的成骨分化。使用定量逆转录聚合酶链反应鉴定标记基因。 MSC在符合GMP的培养基中扩增产生的活细胞符合MSC的所有最低标准。附着分析显示,在蛋白浓度为1-5 fmol / µL的情况下,MSC与层粘连蛋白5和I型胶原蛋白具有良好的结合。与塑料相比,层粘连蛋白5培养28天后成骨分化显着增加(P <0.04)。没有观察到基因表达模式的显着差异。我们得出结论,层粘连蛋白5和I型胶原蛋白促进附着,但层粘连蛋白1和层粘连蛋白5促进MSC的成骨分化。这可能会影响未来的临床应用。

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